Size effects of single-walled carbon nanotubes on in vivo and in vitro pulmonary toxicity

Abstract To elucidate the effect of size on the pulmonary toxicity of single-wall carbon nanotubes (SWCNTs), we prepared two types of dispersed SWCNTs, namely relatively thin bundles with short linear shapes (CNT-1) and thick bundles with long linear shapes (CNT-2), and conducted rat intratracheal i...

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Bibliographic Details
Published in:Inhalation toxicology 2015-03, Vol.27 (4), p.207-223
Main Authors: Fujita, Katsuhide, Fukuda, Makiko, Endoh, Shigehisa, Maru, Junko, Kato, Haruhisa, Nakamura, Ayako, Shinohara, Naohide, Uchino, Kanako, Honda, Kazumasa
Format: Article
Language:English
Subjects:
Administration, Inhalation
Alveolar macrophages
Animals
Bronchoalveolar Lavage Fluid - cytology
Bronchoalveolar Lavage Fluid - immunology
Cell Count
Cell Line
Chemokine CCL3 - immunology
gene expression profiles
Gene Expression Profiling
in vitro
in vivo
intratracheal instillation
Lung - drug effects
Lung - immunology
Lung - pathology
Male
Nanotubes, Carbon - toxicity
Rats, Wistar
Reactive Oxygen Species - immunology
single-wall carbon nanotubes
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Summary:Abstract To elucidate the effect of size on the pulmonary toxicity of single-wall carbon nanotubes (SWCNTs), we prepared two types of dispersed SWCNTs, namely relatively thin bundles with short linear shapes (CNT-1) and thick bundles with long linear shapes (CNT-2), and conducted rat intratracheal instillation tests and in vitro cell-based assays using NR8383 rat alveolar macrophages. Total protein levels, MIP-1 expression, cell counts in BALF, and histopathological examinations revealed that CNT-1 caused pulmonary inflammation and slower recovery and that CNT-2 elicited acute lung inflammation shortly after their instillation. Comprehensive gene expression analysis confirmed that CNT-1-induced genes were strongly associated with inflammatory responses, cell proliferation, and immune system processes at 7 or 30 d post-instillation. Numerous genes were significantly upregulated or downregulated by CNT-2 at 1 d post-instillation. In vitro assays demonstrated that CNT-1 and CNT-2 SWCNTs were phagocytized by NR8383 cells. CNT-2 treatment induced cell growth inhibition, reactive oxygen species production, MIP-1 expression, and several genes involved in response to stimulus, whereas CNT-1 treatment did not exert a significant impact in these regards. These results suggest that SWCNTs formed as relatively thin bundles with short linear shapes elicited delayed pulmonary inflammation with slower recovery. In contrast, SWCNTs with a relatively thick bundle and long linear shapes sensitively induced cellular responses in alveolar macrophages and elicited acute lung inflammation shortly after inhalation. We conclude that the pulmonary toxicity of SWCNTs is closely associated with the size of the bundles. These physical parameters are useful for risk assessment and management of SWCNTs.
ISSN:0895-8378
1091-7691
DOI:10.3109/08958378.2015.1026620